S1P₂-Gα₁₂ Signaling Controls Astrocytic Glutamate Uptake and Mitochondrial Oxygen Consumption

Inhibition of glutamate uptake by S1P contrasts with S1P receptor modulator effects. Primary astrocytes were incubated with labeled glutamate, S1P, or respective agonists for 1 h at 37°C. The glutamate uptake assay was performed as described. A, S1P inhibited glutamate uptake by astrocytes in a dose-dependent manner, while the S1P₁-specific agonist, RP001, did not. B, The relative expression of S1P_1-5 (normalized to β-actin) in wild-type primary astrocytes derived from cerebral cortices of P0 pups. C, The S1P_1,5 modulator, BAF312, did not induce glutamate uptake inhibition at the indicated doses. D, The S1P_1,3,4,5 modulator, FTY720-P, induced partial inhibition. A, C, D, Data are from two independent experiments and curve fitting was performed by nonlinear regression. E, Incubation with FTY720-P for 3.5 d, followed by stimulation with S1P, induced glutamate uptake inhibition similar to no FTY720-P pretreatment controls. Data are representative of three independent experiments. Error bars indicate (mean ± SD). Statistics are calculated by two-way ANOVA performing Sidak’s multiple comparisons test (***p < 0.0005, **p < 0.005; ns, not significant).

Glutamate uptake inhibition is not eliminated in S1P₃-null and astrocyte-specific (As)-S1P₁/S1P₃-double-null astrocytes. Primary astrocytes from As-S1P₁, S1P₃, and As-S1P₁/S1P₃ receptor-null mice were incubated with labeled glutamate and S1P for 1 h at 37°C. A, Glutamate uptake in As-S1P₁^−/− astrocytes exhibited a slight left shift (decrease in glutamate uptake) compared with littermate controls. S1P₃^−/− (B) and As-S1P₁/S1P₃^−/− (C) astrocytes exhibited control levels of glutamate uptake. Data in each panel are from three independent experiments. Curve fitting was performed by nonlinear regression.

Pharmacological inhibition of S1P₂, but not S1P₁ or S1P₃, eliminates astrocytic inhibition of glutamate uptake by S1P. Primary astrocytes were preincubated (A) with or without 10 μM VPC23019, an antagonist for S1P₁ and S1P₃, for 45 min, (B) 10 μM JTE 013, an S1P₂ antagonist, for 30 min, (C) 200 ng/mL PTX overnight, and (D) 10 μM Y27632 for 30 min at 37°C followed by incubation with or without 20 nM S1P for 1 h. Glutamate uptake assays were performed as described. Data in each panel are representative of two independent experiments (n = 3 or 4). Error bars represent mean ± SD; ns, not significant; **p < 0.005, ***p < 0.001, two-way ANOVA with Sidak’s multiple comparisons test.

Genetic removal of S1P₂ or Gα₁₂ downstream signaling reduces astrocytic glutamate uptake inhibition by S1P. Primary astrocytes from S1P₂-null or Gα₁₂-hemizygous-null mice were incubated with labeled glutamate and S1P for 1 h at 37°C. Glutamate uptake in S1P₂^−/− (A) and Gα₁₂^+/− (B) astrocytes exhibited a right shift (increase in glutamate uptake) when compared with controls. Data in each panel are from three independent experiments. Curve fitting was performed by nonlinear regression.